Journal of the Mass Spectrometry Society of Japan 44 巻, 6 号

質量分析法を応用した高感度赤外分光法とそのクラスター科学への適用

The combination of IR-UV double resonance spectroscopy and TOF mass spectrometry enables us to observe the vibrational spectrum of trace molecules or clusters with very high sensitivity and mass selectivity. The molecule in a specific energy level is monitored by REMPI (Resonance Enhance Multi-Photon Ionization) mass spectrometry. The infrared spectrum is observed as a depletion of the ion signal of the specific mass which is induced by the absorption of the infrared laser. The details of the spectroscopic technique and the recent works on the hydrogen bond interactions in the clusters are reviewed.

高速粒子による衝突活性化

Collisional activation of the matter induced by the bombardment of the fast particle is summarized. The particle with the velocity higher than the Bohr velocity (transit time through 5A shorter than 2.5×10^-16s) experiences the electronic stopping power when it passes through the matter and induces dense electronic excitations and ionizations which results in the heavy sputtering of the matter. This kind of activation is usefully applied in the PDMS. When the particle velocity becomes lower than the Bohr velocity, the energy is mainly deposited to the matter by the nuclear stopping power, i.e., energy loss is governed by the screened Coulombic collisions of the atoms giving rise to the momentum transfer to the target nuclei. When the transit time of the particle through 5A is between 2.5×10^-16-10^-14 s, the electronic excitation and ionization take place by the collision. These phenomena are fully utilized in the FAB/SIMS and CID techniques. With the transit time in the range of 10^-14-2.5×10^-13s, the velocity is not high enough for the electronic excitation and the particle loses its energy mainly by the vibrational and phonon excitation of the target. This range of the velocity corresponds to that of the massive cluster impact ionization. With the velocity equal to or lower than 2.5×10^-13s, the energy of the incident particle is consumed mainly by the phonon excitation and the collision results in the modest heating of the colliding interface between the projectile and the target. This range of the velocity is successfully used in the ionized cluster beam technique developed by Takagi of the Kyoto University.

放電型サーモスプレイ方式高速液体クロマトグラフィー/質量分析法を用いた同位体希釈法による血清中有機成分の定量

We review recently developed isotope dilution methods using discharge-assisted thermospray (plasmaspray) liquid chromatography/mass spectrometry (LC/MS) for determination of total cholesterol, glucose, creatinine, and urea in human serum. We have optimized the analytical conditions and discussed the analytical performances of the LC/MS methods. With an optimal conditions, the relative standard deviation of LC/MS methods was between 0.5 and 1.3%. We could conclude that the LC/MS method has the advantage in its simplicity of sample preparation, compared with the GC/MS, and could be a useful technique in IDMS analysis.

Molecular Mass Measurement of Hydrophobic and Aggregative Virus Proteins to Confirm Sequence Variation and Post-translational Modification by Electrospray Ionization and Array Detection

Molecular mass measurements have been studied of outer capsid proteins (P8, -46 kDa) of rice dwarf virus (RDV) by electrospray ionization (ESI) and array detection on a high performance magnetic sector instrument. P8 proteins were highly hydrophobic and aggregative and, therefore, hardly soluble in ESI solvents. Use of an array detector was essential to compensate for the extremely low concentration of solubilized P8 proteins. Extensive tailing of the peak profiles of multiply charged proteins made it difficult to determine their center of gravity representing relative molecular masses (M_r). In stead of M_r, top positions of unresolved peak profiles were utilized which gave molecular masses of the most abundant isotope ions (M_a) at a precision of 0.002%. Precise M_a of P8 proteins suggested the presence of an yet unknown post-translational modification, which was identified as N-terminal acetylation by the sequence analysis of V8-protease digests by FAB-MS/MS. Further, a small difference in M_a (12.3±2.1 Da) between P8 proteins from the ordinary (RDV-O) and the severe (RDV-S) strains of RDV allowed the confirmation of the strain specific amino acid substitution predicted by nucleotide sequencing. The applicability of ESI-MS in combination with array detection was demonstrated for less soluble proteins of biological importance.